Affiliation:
1. Department of Medicine, University of Western Australia, Queen Elizabeth II Medical Centre, Perth, Australia
2. Western Australian Research Institute for Child Health, Princess Margaret Hospital for Children, Perth, Australia
Abstract
1. Platelet-activating factor is a putative mediator of inflammation in asthma and the enzyme acetyl-CoA:lyso-platelet-activating factor acetyltransferase appears to be important in regulating platelet-activating factor production by leucocytes. To determine whether there are differences in acetyl-transferase activity between asthmatic patients and normal subjects, enzyme activity was assayed in neutrophil lysates from atopic asthmatic patients (n = 20), aspirin-sensitive asthmatic patients (n = 12) and healthy, non-atopic, non-asthmatic control subjects (n = 20), both basally and after stimulation with the calcium ionophore A23187.
2. For a range of acetyl-CoA concentrations, acetyl-transferase activity (nmol of [acetyl-3H]PAF min−1 mg−1 of protein) in unstimulated neutrophils from atopic asthmatic patients was significantly higher than that for normal subjects (P = 0.038) and the mean Vmax. for atopic asthmatic patients [18.4 (SD 6.9) nmol min−1 mg−1 of protein] was significantly greater than that for the control subjects [14.9 (SD 4.6) nmol min−1 mg−1 of protein P <0.05]. The mean Vmax. for aspirin-sensitive asthmatic patients [15.9 (SD 6.9) nmol min−1 mg−1 of protein] was not significantly different from that for the normal subjects.
3. The mean ratio Vmax. stimulated/ Vmax. unstimulated for acetyltransferase from atopic asthmatic patients (1.71, SD 0.45) was significantly less than that for the normal subjects (2.13, SD 0.63, P <0.05), suggesting that acetyltransferase from atopic asthmatic patients was less sensitive to stimulation with A23187 in vitro. The mean ratio Vmax. stimulated/ Vmax. unstimulated for aspirin-sensitive asthmatic patients (2.05, SD 0.71) was not significantly different from that for the normal subjects.
4. Vmax. stimulated was significantly correlated with Vmax. unstimulated in atopic asthmatic patients (P = 0.0001) and aspirin-sensitive asthmatic patients (P = 0.012), but not in normal subjects (P = 0.071).
5. These results suggest that, in atopic asthmatic patients, neutrophils may be subject to chronic priming in vivo for increased acetyltransferase activity and capacity for platelet-activating factor synthesis. In these patients the increased platelet-activating factor production may be contributing significantly to the degree of inflammation associated with their asthma.
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